Fluorescence polarization as a tool for the determination of deoxynivalenol in wheat

C. Maragos, M. Jolley, M. Nasir
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引用次数: 33

Abstract

The mould Fusarium graminearum is found worldwide as a pathogen of cereal grains, in particular of wheat and maize, and it produces a mycotoxin known as deoxynivalenol (DON or vomitoxin). Each year, the presence of this compound and related trichothecenes causes substantial losses to agricultural productivity. Rapid methods for the measurement of the toxin in grains are required to monitor and divert effectively contaminated grain from the food supply. A fluorescence polarization (FP) immunoassay using a previously described monoclonal antibody for DON was developed. The assay was based on the competition of unlabeled DON from a sample with a fluorescently tagged DON, DON-fluorescein (DON-FL), for a DON-specific monoclonal antibody in solution. The FP of the tagged DON was increased upon binding with the antibody. In the presence of free toxin, less of the DON-FL was bound and the polarization signal was decreased. The assays were very simple to perform, requiring only mixing of an aqueous extract of wheat with the DON-FL and antibody. The sensitivity of the assay was strongly dependent upon the time between mixing of the sample with the tracer and measurement of the fluorescence polarization, with midpoints for the competition curves ranging from 0.03 µgml-1 with a 15-s incubation to >1 µgml-1 with a 12-min incubation. Samples of wheat naturally contaminated with DON were evaluated by FP and by an HPLC-UV method, with a good correlation (r 2 = 0.97). Although the FP method tended to overestimate DON slightly in the wheat samples, by ˜20%, the assay was easy to use and very useful for the screening of wheat.
荧光偏振法测定小麦中脱氧雪腐镰刀菌醇
稻谷镰刀菌是谷物,特别是小麦和玉米的一种病原体,在世界各地都有发现,它产生一种真菌毒素,称为脱氧雪腐镰刀菌醇(DON或呕吐毒素)。每年,这种化合物和相关的毛霉烯的存在对农业生产力造成重大损失。需要快速测定谷物中毒素的方法,以便有效地监测和转移受污染的粮食。利用先前描述的DON单克隆抗体,开发了一种荧光极化(FP)免疫分析法。该分析是基于样品中未标记的DON与荧光标记DON-荧光素(DON- fl)在溶液中竞争DON特异性单克隆抗体。标记DON的FP与抗体结合后增加。在游离毒素存在的情况下,DON-FL的结合量减少,极化信号减弱。该检测操作非常简单,只需要将小麦的水萃取物与DON-FL和抗体混合。该检测的灵敏度强烈依赖于样品与示踪剂混合和荧光偏振测量之间的时间,竞争曲线的中点范围为0.03µgml-1(孵育15 s)到>1µgml-1(孵育12 min)。用荧光定量法和高效液相色谱-紫外分光光度法对天然污染的小麦样品进行评价,相关性较好(r 2 = 0.97)。虽然FP法在小麦样品中倾向于略微高估DON,约为20%,但该方法易于使用,对小麦的筛选非常有用。
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